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体外肝细胞分化:培养的胎鼠肝细胞中酪氨酸转氨酶表达的起始

Hepatocyte differentiation in vitro: initiation of tyrosine aminotransferase expression in cultured fetal rat hepatocytes.

作者信息

Shelly L L, Tynan W, Schmid W, Schütz G, Yeoh G C

机构信息

Department of Physiology, University of Western Australia, Nedlands.

出版信息

J Cell Biol. 1989 Dec;109(6 Pt 2):3403-10. doi: 10.1083/jcb.109.6.3403.

Abstract

A fetal rat hepatocyte culture system has been used to study the molecular mechanisms of tyrosine aminotransferase (TAT) gene expression during development. It has previously been shown that TAT activity can be detected in 19-d, but not 15-d, gestation hepatocytes on the first day of culture (Yeoh, G. C. T., F. A. Bennett, and I. T. Oliver. 1979. Biochem. J. 180:153-160). In this study enzyme activity, synthesis, and mRNA levels were determined in hepatocytes isolated from 13-, 15-, and 19-d gestation rats maintained in culture for 1, 2, or 3 d and exposed to dexamethasone. TAT expression is barely detectable in 13-d gestation hepatocytes even after 3 d in culture. Hepatocytes isolated from 15-d gestation fetuses have undetectable levels of enzyme activity and synthesis on the first day of culture; both can be assayed by days 2 and 3. TAT mRNA levels in these hepatocytes, measured by hybridization with a specific cDNA, increase substantially during culture. TAT activity, synthesis, and mRNA are evident on the first and subsequent days of culture in 19-d gestation hepatocytes. Transcription measurements in isolated nuclei indicate that the increase in TAT mRNA in 15- and 19-d gestation hepatocytes is associated with an increase in transcription of the gene. Immunocytochemical studies demonstrated that the increase in TAT expression correlated with an increase in the proportion of hepatocytes expressing the enzyme, rather than a simultaneous increase in all hepatocytes. These results support the proposal that a subpopulation of 15-d fetal hepatocytes undergo differentiation in culture with respect to TAT.

摘要

一种胎鼠肝细胞培养系统已被用于研究发育过程中酪氨酸转氨酶(TAT)基因表达的分子机制。先前的研究表明,在培养的第一天,妊娠19天的肝细胞中可检测到TAT活性,但妊娠15天的肝细胞中则检测不到(Yeoh, G. C. T., F. A. Bennett, and I. T. Oliver. 1979. Biochem. J. 180:153 - 160)。在本研究中,测定了从妊娠13天、15天和19天的大鼠分离得到的肝细胞在培养1、2或3天并暴露于地塞米松后的酶活性、合成及mRNA水平。即使培养3天后,妊娠13天的肝细胞中TAT表达仍几乎检测不到。从妊娠15天的胎儿分离得到的肝细胞在培养第一天酶活性和合成水平均检测不到;在第2天和第3天均可检测到。通过与特异性cDNA杂交测定,这些肝细胞中的TAT mRNA水平在培养过程中大幅增加。妊娠19天的肝细胞在培养的第一天及随后几天TAT活性、合成及mRNA均很明显。分离细胞核中的转录测量表明,妊娠15天和19天的肝细胞中TAT mRNA的增加与该基因转录的增加相关。免疫细胞化学研究表明,TAT表达的增加与表达该酶的肝细胞比例增加相关,而非所有肝细胞同时增加。这些结果支持了这样一种观点,即妊娠15天的胎儿肝细胞亚群在培养过程中就TAT而言发生了分化。

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